. Author manuscript; available in PMC: 2023 Jul 13.

Published in final edited form as: Adv Ther (Weinh). 2019 Sep 30;2(12):1900133. doi: 10.1002/adtp.201900133

Table 1.

Comparisons of different transfection techniques for cell therapies

	Fugene^® (DNA:Reagent = 1:2.5, 30 uL of reagent-DNA mixture)	Viral (lentivirus with ubiquitin promoter, MOI = 10)	Bulk electroporation (Biorad, 1000 μF, 500 V, 30 s)	Nano-electro injection (NEI) system (30 V, 40 Hz, 200 μs, 2 min)
Net efficiency (E_net)	11.2%	19.5%	16.5%	23.8%
Measured cell doubling time (t_d)⁺	46.8 hr (^**)	53.1 hr (^**)	50.6 hr (^**)	40.0 hr (n.s.)
# days to reach N_final (D)	30.1	32.4	31.6	23.9

Starting cell # (N₀) = 0.2*10⁶ and final cell # (N_final) = 10⁹

${N_{f i n a l} = N}_{0} * E_{n e t} * 2^{n}$ , where n is the number of cell divisions. Based on this calculation, the ‘n’ value for Fugene, viral, Biorad and NEI are 15.4, 14.6, 15.0 and 14.4 respectively.

⁺

tracked for first 4 days after transfection and assuming the value remains unchanged. Our control cells without any transfection treatment doubled every 36.4 hr on average (Table S5).

^**

/n.s. indicates p-value <0.001/non-significant respectively compared to control cells, with starting 0.2*10⁶ cells in each condition.

$D = n * t_{d}$